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Detection and purification of proteins are the core methods in life science experiments. The biotin-avidin interaction is often used to detect or purify proteins because of its high binding affinity. 1 and 2 are biotinylation reagents containing both a linker and an N-hydroxysuccinimidyl ester (NHS) moiety and are pre-weighed in suitable amounts for protein biotinylation. They can biotinylate proteins by reacting with amino groups (-NH2) of proteins and by forming amide bonds at pH between 7 and 9. Below is the direction for use.
Preparation: It is recommended to prepare a 10 mM biotinylation solution. In order to efficiently biotinylate a sample, biotinylation solution should be used at a 15-fold molar excess over the amount of amine-containing protein. Here shows the calculation of the 10 mM biotinylation solution amount. Calculate Example: A μL of 10 mM biotinlation solution for biotinylation 2 mg IgG (150,000 M.W.)
2 [mg IgG] × 10-3 [g/mg] × 1/150,000 [mol/g] × 15 [fold] = A [μL of 10 mM biotinylation solution] × 10-6 [L/μL] × 10 [mmol/L] × 10-3 [mol/mmol]
A = 20 [μL of 10 mM biotinylation solution]
Direction for Use
Bring 1, 2 to room temperature and dissolve 2 mg of 1 in 350 μL of DMSO or DMF, or 2 mg of 2 in 400 μL of PBS to prepare a 10 mM biotinylation solution.
Dissolve the sample (1-10 mg/mL) in an appropriate buffer with pH between 7 and 9 such as PBS. Do not use buffers including amines (such as Tris).
Add A μL (calculated above) of 10 mM biotinylation solution to the sample solution and incubate the mixed solution for 30 min at room temperature.
Remove unreacted and hydrolyzed reagent by a desalting column or dialysis.
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